Eruca sativa and Diplotaxis tenuifolia - ACS Publications - American

Apr 29, 2014 - This review highlights how breeders and processors of rocket ... Plant breeders are increasingly looking to new technologies such as HP...
0 downloads 0 Views 3MB Size
Review pubs.acs.org/JAFC

Glucosinolates, Myrosinase Hydrolysis Products, and Flavonols Found in Rocket (Eruca sativa and Diplotaxis tenuifolia) Luke Bell* and Carol Wagstaff Department of Food and Nutritional Sciences and the Centre for Food Security, University of Reading, Whiteknights, Reading, Berkshire RG6 6AH, United Kingdom ABSTRACT: Rocket species have been shown to have very high concentrations of glucosinolates and flavonols, which have numerous positive health benefits with regular consumption. This review highlights how breeders and processors of rocket species can utilize genomic and phytochemical research to improve varieties and enhance the nutritive benefits to consumers. Plant breeders are increasingly looking to new technologies such as HPLC, UPLC, LC-MS, and GC-MS to screen populations for their phytochemical content to inform plant selections. This paper collates the research that has been conducted to date in rocket and summarizes all glucosinolate and flavonol compounds identified in the species. The paper emphasizes the importance of the broad screening of populations for phytochemicals and myrosinase degradation products, as well as unique traits that may be found in underutilized gene bank resources. This review also stresses that collaboration with industrial partners is becoming essential for long-term plant breeding goals through research. KEYWORDS: Brassicaceae, isothiocyanates, plant breeding, indoles, nitriles



Gomez-Carneros,26 Keum et al.,27 D’Antuono et al.,28 EgeaGilbert et al.,29 Degl’Innoocenti et al.,30 Bjorkman et al.,31 and Jeffery et al.32

INTRODUCTION In recent years, several species of minor leafy crops have risen to prominence as potentially important commercial and edible species. One example is rocket, which has quickly gained popularity in the Western diet. Originally found as an obscure crop in Mediterranean and Middle Eastern countries, rocket has become popular largely due to the pungent aromas and tastes associated with it. Glucosinolates (GSLs)/isothiocyanates (ITCs) and flavonols derived from many species1−4 have been shown to impart significant protection against cancer and heart disease.4−11 In Western countries, diets are generally lacking in fruits and vegetables. Despite government initiatives (such as the “5-a-day” campaign in the United Kingdom and the United States), these diseases are increasingly leading to premature deaths.12 Plant breeders aim to maximize levels of such beneficial compounds, but with little genomic information about rocket species presently available, this is a formidable task. This review will give an overview of research in rocket, an outbreeding crop, and how breeders and processors can utilize it to enhance beneficial compounds.



A distinction should be made that both Eruca and Diplotaxis species have overlapping characteristics and that one can be easily mistaken for the other by the untrained eye and/or before a certain level of maturity has been reached.28 It is also arguable that D. tenuifolia is the least “wild” of the two species even though the common name is “wild rocket”. It is featured and favored in commercial products and breeding programs and is likely to be more domesticated than Eruca species as a result. Diplotaxis varieties are generally uniform phenotypically, with Eruca varieties being more diverse in this respect.23 No direct genomic evidence has been presented in the literature to suggest one species is any more or less genetically variable than the other. Variability in GSL data seems to support the hypothesis that Diplotaxis species are more “wild”,33 although it is not conclusive, as only a relatively small number of cultivars have been tested. This is a point that needs clarification through research and extensive breeding, as neither species can be considered fully domesticated.29 For example, germination rates are variable, reproductive organs are typically small, seedpods shatter and disperse freely (rather than staying on the plant), and physical defenses such as leaf hairs are still present in many commercial varieties.34



ROCKET SPECIES Rocket (also known as arugula, rucola, and roquette) is a leafy vegetable crop that has gained substantial popularity across the world, particularly over the past 15 years.13−16 Two main species are predominantly farmed as salad crops; these are Eruca sativa (“salad” or “cultivated” rocket; sometimes referred to as Eruca vesicaria subsp. sativa) and Diplotaxis tenuifolia (“wild” rocket). Both species share a peppery taste and aroma that is very distinctive.17 They have been reported to contain high levels of vitamin C, GSLs, flavonols, and phenolics.18−25 These are all known to have both antioxidant and anticancer properties and are also implicated in lowering the risk of cardiovascular and cognitive diseases. For excellent information on these beneficial effects and their underlying causes, see Drewnowski and © 2014 American Chemical Society

TAXONOMY AND DOMESTICATION

Received: Revised: Accepted: Published: 4481

October 6, 2013 April 28, 2014 April 29, 2014 April 29, 2014 dx.doi.org/10.1021/jf501096x | J. Agric. Food Chem. 2014, 62, 4481−4492

Journal of Agricultural and Food Chemistry

Review

Figure 1. Glucosinolate−myrosinase reaction and some of the subsequent compounds produced under different conditions, such as pH and the influence of epithiospecifier proteins (ESP). Adapted from Zhang9 and Hall et al.185



PHYTOCHEMICALS IN ERUCA SATIVA AND DIPLOTAXIS TENUIFOLIA: TYPES AND STRUCTURES Glucosinolates. GSLs are β-thioglucoside N-hydrosulfates that are responsible for the sharp and bitter-tasting flavors found in cruciferous vegetables.35,36 In combination with the enzyme myrosinase (thioglucoside glucohydrolase, EC 3.2.1.147), GSLs are hydrolyzed to create isothiocyanates, nitriles, thiocyanates, epithionitriles, indoles, oxazolidine-2-thiones, cyanopithioalkanes, ascorbigens, goitrogens, and epithioalkanes37−49 (see Figure 1). Many of these hydrolysis products have antibacterial, antifungal, and insect-repellant effects.50−55 GSLs and ITCs are being increasingly used as “biofumigants” to suppress soilborne pathogens, nematodes, and weeds. Some of the volatile products have the opposite effect of attracting species that can tolerate high GSL concentrations, such as types of ovipositing insects.56,57 The conditions under which hydrolysis of GSLs occurs will affect the respective proportions of the chemicals produced; pH, iron ions, thiol ions, temperature, and hydration play a particularly prominent role in this process in vivo.58 The separation of GSLs in specialist “S-cells” from myrosinase in myrosin cells means that the two components come into contact only upon tissue disruption, for example, when damaged via chewing or digestion.59−69 It is the biological activity of the ITC hydrolysis products in humans that is of most interest in rocket.50 GSLs can be hydrolyzed within the intestinal tract by gut microflora that are known to have specific myrosinase activity,70−73 but the efficacy of their action is not yet well determined. GSL concentrations can vary and change over time depending on environmental conditions and stress.7 Other factors affecting GSL profiles include plant age, organ type, developmental stage, ambient air temperature, level of water stress, photoperiod, agronomic practice, degree of wounding, and geographical origin of the variety/species.74−81 These can often affect the profiles of all phytonutrients contained within tissue, not just GSLs,82 and they are all factors that plant breeders aim to mitigate through development of genetically advanced and uniform breeding lines. GSLs and the ITC derivatives have been an integral part of the human diet for millennia because of their presence in the family Brassicaceae.64−66,83−89 GSLs are evolutionarily recent

secondary metabolic products, having arisen 10−15 million years ago,90,91 acting to prevent pathogen attack and dissuade herbivory. They are known in only a few angiosperm families of the order Brassicales, which includes the Brassicaceae,92−100 and of which Eruca and Diplotaxis are members. A study by Pasini et al.33 of 37 rocket accessions (Diplotaxis and Eruca) showed that GSL profiles were all very similar, regardless of the species. In total, 12 GSL compounds were found across all accessions; Table 1 illustrates all known GSL compounds identified to date in rocket. These include 4-mercaptobutyl GSL (glucosativin),21 4-methylthiobutyl GSL (glucoerucin),101 and 4-methylsulfinylbutyl GSL (glucoraphanin),28 which constitute the three most abundant GSLs in rocket. Flavonols. Flavonols are diphenylpropanes (C6−C3−C6)102 and are another important group of chemicals found within rocket species. Flavonols in rocket are found with sugar conjugates and typically occur in relatively large quantities.103 The aglycones found (such as quercetin and kaempferol) are glycosylated and acylated, which in turn affects their biological properties.18 A study by Martı ́nez-Sań chez et al.18 identified over 50 different flavonol compounds across four different species. Watercress, mizuna, and two species of rocket were all found to accumulate very different compounds within their leaves and in varying quantities. Wild rocket showed high levels of quercetin-3,3′,4-triglucosyl (43.5 mg 100 g−1 fw), and salad rocket had mostly kaempferol-3,4′-diglucosyl (97.8 mg 100 g−1 fw). The group also showed a correlation between quercetin derivatives and high antioxidant activity, despite the significant variations seen between species. Studies conducted on rocket tissues have identified significant concentrations of polyglycosylated flavonols. The core aglycones of these are kaempferol, quercetin, and isorhamnetin;102 Table 2 provides an up-to-date list of all flavonol compounds identified in rocket. Martı ́nez-Sanchez et al.18 showed that Eruca species accumulate kaempferol derivatives, whereas D. tenuifolia accumulates predominantly quercetin instead, meaning that the two chemicals could be used as identification markers between the two species.104 Isorhamnetin aglycones are common to both species but typically in much lower concentrations.33 The specific aglycones also impart various degrees of antioxidant activity. For example, quercetin derivatives have a higher activity than kaempferol and isorhamnetin. The differences in structure 4482

dx.doi.org/10.1021/jf501096x | J. Agric. Food Chem. 2014, 62, 4481−4492

Journal of Agricultural and Food Chemistry



Review

PHYTOCHEMICALS AND THE RELATIONSHIP WITH QUALITY: TASTE AND AROMA It is thought that the presence of glucosativin, glucoerucin, and their hydrolysis products within rocket leaves is what gives

(the arrangement of hydroxyl groups and glycosylation) affect antioxidant activity by allowing the molecules to act as hydrogen/electron donors, single-oxygen scavengers, or reducing agents.105

Table 1. Intact Glucosinolates Identified within Leaves of Rocket, Eruca and Diplotaxis Species, by LC-MS (Negative Ion Mode)

4483

dx.doi.org/10.1021/jf501096x | J. Agric. Food Chem. 2014, 62, 4481−4492

Journal of Agricultural and Food Chemistry

Review

Table 1. continued

x

Standard GSL molecule according to IUPAC nomenclature.

them a characteristic flavor.44 Many of the health beneficial GSLs and ITCs are thought to be responsible for strong tastes that some consumers find repellant.106 It seems that to many people, these compounds contribute very little to a pleasurable eating experience and are actively avoided.83 Conversely, however, some people prefer these strong tastes and aromas and will actively seek to consume rocket when it is available. Growers in Italy often prefer the subsequent cuts because of the more intense tastes and aromas that are produced,107 and some will even “sacrifice” the first cut in favor of the subsequent leaf growth. This highlights a divide between consumers that may be indicative of underlying genotype(s) for taste perception and preference.

The breeding process in rocket varieties to date has effectively made the species “milder” in taste when compared to plants that grow naturally in the wild. Whether this has been intentional or as a result of selecting for other unrelated traits (such as leaf morphology) is debatable. Some recent commercial varieties have been bred for a “hotter” taste, such as ‘Wildfire’, by Tozer Seeds (Surrey, UK). A study by Pasini et al.17 demonstrated how breeding for sensory traits could be achieved by highlighting which glucosinolates contribute to specific taste and aroma elements in rocket. It was found that progoitrin/epiprogoitrin is responsible for bitter taste attributes, despite being only a minor component of the overall GSL profile of rocket (4.3−11.4% of total 4484

dx.doi.org/10.1021/jf501096x | J. Agric. Food Chem. 2014, 62, 4481−4492

Journal of Agricultural and Food Chemistry

Review

Table 2. Flavonol Compounds Identified in Leaves of Eruca and Diplotaxis Species by LC-MS (Negative Ion Mode) flavonol compounda

Erucab

Diplotaxisb

mass parent ion

I 3,4′-diGlc I 3-Glc K 3-(2-Sinp-Glc)-4′-Glc K 3,4′-diGlc K 3-Glc Q 3-Glc

X X X X X X

X

639 477 817 609 447 463

K 3-diGlc-7-Glc K 3-Sinp-triGlc-7-Glc Q 3,4′-diGlc-3′-(6-Caf-Glc) M Q R

X X

X

X X X X

MS2 spectrum ions (signature ion in bold) 477

refs 18, 33

285 301

771 1139 949 317 301 609

609 977, 771, 609, 429 787, 625, 463, 301 151 151 300

33

189

Q 3-(2-Caf-Glc)-3′-(6-Sinp-Glc)-4′-Glc Q 3-(2-Mcaf-Glc)-3′-(6-Sinp-Glc)-4′-Glc

X X

1155 1185

993, 831, 787, 669, 625, 463, 301 1023, 817, 669, 655

18, 25

Q 3-(2-Fer-Glc)-3′-(6-Fer-Glc)-4′-Glc Q 3-(2-Fer-Glc)-3′-(6-Sinp-Glc)-4′-Glc

X X

1139 1169

977, 639, 463 1007, 831, 669, 639, 463, 301

18, 25, 33

Q Q Q Q Q Q

X X X X X X

1199 787 963 979 933 993

1037, 831, 669, 463, 301 625, 463, 301 801, 639, 463, 301 817, 655, 463, 301 771, 609, 463, 301 831, 669, 463, 301

18, 25, 33

3-(2-Sinp-Glc)-3′-(6-Sinp-Glc)-4′-Glc 3,3′,4-triGlc 3,4′-diGlc-3′-(6-Fer-Glc) 3,4′-diGlc-3′-(6-Mcaf-Glc) 3,4′-diGlc-3′-(6-p.Coum-Glc) 3,4′-diGlc-3′-(6-Sinap-Glc)

a Abbreviations: Caf, caffeyol; Mcaf, methoxycaffeyol; p.Coum, p-coumaroyl; Fer, feruloyl; Sinp, sinapoyl; Glc, glucoside; Q, quercetin; K, kaempferol; I, isorhamnetin; M, myricetin; R, rutin. bCompound positively identified in species.

very strong antigenotoxic effects of E. sativa extracts,13 which is in agreement with other Brassicaceae studies.114,115 Identifying specific cultivars of rocket with elevated levels of erucin and glucoraphanin would be an important first step in developing superior varieties from a human nutrition standpoint. The results of GSL/ITC research prompted an investment in broccoli breeding in the past decade. A similar concerted effort could be made for rocket, which contains similar compounds that are potentially just as efficacious in humans.116 Erucin, for example, has been shown to have a very similar, and even superior, biological activity to that of sulforaphane.117 One paper has specifically demonstrated that the concentration of rocket ingested in an average daily diet is significant enough to impart a cancer preventative effect.13 The metabolism of ITCs in humans via the mercapturic acid pathway has been investigated. ITCs are conjugated with glutathione and degraded by N-acetylation, initiating an increase of phase II detoxification enzymes; see Figure 3 for the detailed pathway breakdown of erucin.113 Nitriles. Along with ITCs, nitriles are the most abundant bioactive compounds produced by GSL hydrolysis.116 The hydrolysis of glucoraphanin, for example, yields predominantly sulforaphane and sulforaphane nitrile. The ratio in which the two are formed depends greatly upon the environmental conditions and the plant cultivar that is used.117 A low-pH medium tends toward the formation of nitriles, whereas high pH forms ITCs.118,119 The presence of thiol and iron ions favors nitriles, and high temperature and hydration produce more ITCs.120,121 This can have substantial consequences for any potential health benefits that might be imparted by the consumption of rocket.119 The nitrile form is approximately 3 orders of magnitude less efficacious than the ITC in inducing quinone

GSL concentration). The perceived pungency of leaves was positively related to the overall GSL content of accessions, and the levels of glucoraphanin negatively contributed to the typical “rocket” flavor. The study also highlighted an important difference between rocket and other Brassica sensory studies108 in that bitterness was perceived as a favorable characteristic according to panelists. The flavonol compound kaempferol-3(2-sinapoylglucoside)-4′-glucoside also significantly and positively contributed to flavor attributes in Eruca accessions. This would indicate that GSL compounds are not totally responsible for flavor in rocket. The study itself stopped short of saying how or if the information obtained would be used in breeding programs, but with study into rocket flavor components, milder (and/or stronger) varieties could be bred more efficiently once the responsible compounds are properly identified.26



HEALTH-PROMOTING PROPERTIES OF GLUCOSINOLATE−MYROSINASE PRODUCTS AND FLAVONOLS OF ROCKET Isothiocyanates. ITC hydrolysis products have been identified in rocket,45 such as 4-(methylthio)butyl ITC (erucin),109,110 which is known to show antiproliferative activity in human lung carcinoma A549 cells, hepatoma (HepG2) cells, colon cancer cells, prostate cancer cell lines (PC3, BPH-1, and LnCap), and leukemia cells.111 Erucin is a structurally reduced analogue of sulforaphane (which is predominantly found in broccoli) and has shown promising anticancer properties in vitro (e.g., antiproliferation of human erytroleukemic K562 cells).112 Research into the chemopreventative and antigenotoxic nature of ITCs has shown promising results113 (see Figure 2). Other studies involving chemically induced genotoxicity have shown 4485

dx.doi.org/10.1021/jf501096x | J. Agric. Food Chem. 2014, 62, 4481−4492

Journal of Agricultural and Food Chemistry

Review

Figure 2. Pathways of documented ITC action in tumorigenic cells. See Wu et al.113 for a detailed review of the roles ITCs play in cancer prevention.

programmed cell death in prostate, breast, and osteocarcinoma cell lines139 and G1 cell cycle arrest in breast and prostate cancer cell lines.140,142,143 It is these cytostatic effects on cell proliferation that have been suggested as the mechanism responsible for the lack of apoptosis effects in indoles.141 Using information on GSL content in rocket, the ITC and indole effects can be potentially maximized in new varieties and be of greater benefit to human health when considered in tandem, rather than separately.127 Oxazolidine-2-thiones and Goitrogens. The hydrolysis of β-hydroxy-alkyl GSL compounds (e.g., progoitrin; a minor GSL in rocket) can produce oxazolidine-2-thiones such as goitrin (5-vinyloxazolidine-2-thione).142−148 It is these compounds that are largely attributed to the thyroid condition of goiter in mammals,149 but the action of microflora in the gut is thought to mediate the problems associated with high oxazolidine-2-thione intake.150−153 That being said, oxazolidine2-thiones interfere with thyroxine synthesis154 and are therefore likely to have an adverse biological effect regardless of gut microflora action or bodily iodine status.3 A study by Nishie and Daxenbilcher155 showed that these compounds are not teratogenic or embryotoxic, however. These molecules contribute significantly to the bitter taste of rocket that some people perceive quite strongly.154 The detection of these compounds may be mediated in a similar genetic fashion as PROP (propylthiouracil), for example.155,156 By using phytochemical data in rocket breeding programs these oxazolidine-2-thione components could be reduced, potentially improving consumer acceptance (depending on the target consumer) and avoiding any possible adverse health effects associated with overconsumption. Ascorbigens. Ascorbigens are formed via the reaction of indole-3-carbinol and 3,3′-diindolymethane with ascorbic acid in the stomach during myrosinase-catalyzed degradation of indolyl-3-methyl glucosinolates.157,158 In this manner it is

reductase (phase II enzyme) and thus imparts a reduced enzymatic and anticarcinogenic response. Nitriles also compete with ITCs in this induction and reduce potential positive effects further.38 As the ratio of these compounds may depend on plant variety, care must be taken in rocket breeding when plants are selected for GSL content, as this may not be reflective of the bioactives produced in subsequent hydrolysis reactions.122 Other underlying genetic factors may influence which degradation pathway is taken.123,124 Indoles. Indoles are the predominant autolysis product of indole glucosinolates such as glucobrassicin, as their ITC counterparts are unstable.85 Glucobrassicin has been detected as a minor GSL in rocket species,33 and the predominant indole species produced is indole-3-carbinol. This compound is known to be cancer-preventative,125,126 particularly in reproductive organs in vitro and in vivo. A condensation product of indole-3carbinol, 3,3′-diindolymethane, is also responsible for beneficial physiological effects. Both compounds have been shown to reduce cell proliferation in breast, prostate, cervical, and colon cancer cell lines. They also show distinct differences from ITCs such as sulforaphane127 and inhibition of tumor development in the stomach, breast, uterus, tongue, and liver of rodents.128−135 Experiments in rodents have shown an increase in drugmetabolizing enzymes in the stomach, liver, and small intestines of individuals consuming both ITCs and indoles. This is suggestive of enhanced detoxification phase II enzymes (such as quinone reductase, glutathione reductase, and glutathione transferase)134 and a mechanism by which these phytochemicals impart chemopreventative effects.135,136 Typically indoles inhibit cell proliferation through cytostatic mechanisms, whereas ITCs induce cytotoxicity within cell lines (at >12.5 μM concentrations), which ultimately leads to increased apoptosis.137,138 This indicates that both types of compound could act and be effective at different stages of cancer development.11 Indoles have been shown to induce 4486

dx.doi.org/10.1021/jf501096x | J. Agric. Food Chem. 2014, 62, 4481−4492

Journal of Agricultural and Food Chemistry

Review

Figure 3. Mercapturic acid pathway of ITC metabolism in the human body. After ingestion of rocket leaves, glucoerucin is hydrolyzed by myrosinase to form erucin. This is released and absorbed in the ileum, where it is transported in the blood to cells around the body. ITCs initiate phase II detoxification enzymes in this pathway and are known to aid in cancer prevention. Adapted from Wu et al.113

thought that ascorbigens have a role in cancer modulation159 via quinone reductase induction.114 As has been highlighted previously, this has important implications for breeding for plant varieties with enhanced chemopreventative effects. Epithioalkanes. Epithioalkanes are formed as part of the myrosinase reaction with GSLs at low pH with epithiospecifier protein and ferrous ions. These GSLs typically have a side chain with a double bond, such as sinigrin.160−163 It is uncertain whether these compounds produce any significant bioactive effect in humans, but the ratio in which they are produced alongside ITCs, nitriles, and indoles may affect on these compounds’ efficacy as anticarcinogens.

Flavonols. The antioxidant and anti-inflammatory function of flavonols in the human diet are well-known and include protecting the colonic epithelium from free radical damage.164−167 They can induce the up-regulation of enzymes (such as cytochrome P450), which may lead to a decreased risk of cancer, cardiovascular disease, immune dysfunction, atherosclerosis, and chronic inflammation.168,169



FACTORS AFFECTING PHYTOCHEMICAL CONTENT Breeding and Cultivation. Rocket has been consistently shown to be a good dietary source for flavonols, GSLs, and antioxidants. However, there can be large differences between 4487

dx.doi.org/10.1021/jf501096x | J. Agric. Food Chem. 2014, 62, 4481−4492

Journal of Agricultural and Food Chemistry

Review

plants of the same germplasm accession due to a combination of genetic and environmental variability. This is probably due to the outbreeding nature of the species104 and a lack of overall uniformity in varieties. Commercial varieties cannot be considered truly domesticated because of this tendency for outcrossing, and the susceptibility of plants to inbreeding depression (a loss of genetic variability due to repeated selfpollination or crossing with a closely related individual). Development of advanced open-pollinating breeding lines (lines that are allowed to cross-pollinate freely in a population of selected individuals), or even F1 hybrids (superior varieties produced by crossing distinctly different, elite inbred lines), could potentially minimize such variation. Throughout the food chain there are many aspects that can have an adverse effect on GSL levels within leaves (Figure 4). These include cultivar choice, cultivation practice, climatic conditions, photoperiod, sulfur and nitrogen availability, harvest date, time spent in storage, temperature of wash water, levels of physical damage to leaves, packaging atmosphere, and food preparation methods.30−32,170−173 Harvesting. Rocket species have the ability to regrow their leaves repeatedly after cutting, which allows for several harvests to take place under optimal conditions.107 In parts of southern Italy, it is not unheard of for up to seven harvests to occur from a single planting. This has obvious cost-saving benefits for growers, but multiple harvests also induce stress responses in rocket that may be detrimental to the flavor and aesthetics of the crop. Stress drives up the production of secondary metabolites such as GSLs and anthocyanins, which will produce very strong, bitter tastes. There are other detrimental effects of multiple harvests; leaves become progressively smaller and more “skeletal” in appearance with each cutting, for example. High anthocyanin levels also affect the color of leaves, turning them an undesirable pink, purple, or red. Color has been found to be one of the most important characteristics consumers look for in rocket,174 and so the loss of fresh appearance can ultimately lead to rejection of crops by supermarkets and processors. Industrial and Culinary Processing. There are five main influences that have been identified as affecting GSL levels during processing.94 These are the action of myrosinase hydrolysis, myrosinase inactivation, the lysis and leaching of GSLs into wash water, thermal degradation of GSLs, and the loss of ascorbic acid, iron, and other enzyme cofactors. Myrosinase inactivation and thermal degradation of GSLs is probably less of an issue in rocket species, as the leaves are not typically cooked. The leaves are not ordinarily frozen, and so freeze−thaw hydrolysis is not likely to be a major factor either. Other factors almost certainly play a significant role in GSL and phytochemical loss in rocket. Verkerk et al.94 highlighted four key areas that affect GSL levels before reaching the end consumer: (1) variety/ cultivar used; (2) storage and packaging (postharvest, postprocessing, and in shops/supermarkets); (3) industrial processing; and (4) consumer preparation methods. If each of these areas can be mitigated through breeding superior varieties, consumers will receive an end product that is of higher nutritive quality and thus provides increased health benefits. Postharvest Storage. Studies on both Diplotaxis and Eruca species have been conducted to determine the effects of postharvest storage conditions on chlorophyll content and respiration rates.15 Both species of rocket have been found to have high respiration rates,107 leading to rapidly impaired

Figure 4. Factors and conditions within the commercial supply chain that affect GSL and flavonol levels within rocket leaves.

visual quality, such as stem browning, tissue yellowing, and general decay.175 Provided initial GSL loss can be mitigated through breeding, ITC formation has been shown to increase over nitrile formation during the storage period.176 Time, temperature, humidity, and atmospheric conditions are all optimized for specific crops within the logistics chain, but these factors are often designed to prevent only visual degradation and not phytochemical breakdown.100 Getting producers, packagers, and transporters to change their current practices to better preserve the health-promoting compounds in rocket would be a difficult task. Treatments and storage conditions are often integrated parts of protocols and procedures, and changing these would require significant testing on a commercial scale. 4488

dx.doi.org/10.1021/jf501096x | J. Agric. Food Chem. 2014, 62, 4481−4492

Journal of Agricultural and Food Chemistry



Review

NEW SELECTION TOOLS FOR BREEDERS Phytochemical Selection. It should not be forgotten that some GSLs and their breakdown products are thought to be toxic, and even carcinogenic, at high concentrations.128 Breeders and researchers should be mindful that more of a certain compound does not necessarily mean “better”.177 Humans seem to be able to tolerate GSLs much better than pigs, rats, and rabbits, for example, but overconsumption of these compounds may have serious health consequences64 as high-dose−effect relationships are as yet unknown in humans.94 Few papers in GSL research (regardless of species) have acknowledged the potential for plant breeders to utilize HPLC/ UPLC/LC-MS/GC-MS methods within breeding programs to “monitor” and select plants for their phytochemical content in this manner. These techniques would provide valuable information on breeding lines relatively rapidly, especially for GSL and flavonol breeding.178 It is not common practice to select rocket plants on the basis of their phytochemical profile at present, but as interest in these compounds increases, it will be necessary for breeders to modify their selection criteria and information sources to remain competitive in the salad vegetable market.94 This has been achieved with ‘Beneforte’ broccoli (Seminis Vegetable Seeds; subsidiary of Monsanto Co., St. Louis, MO, USA; www.beneforte.com) for example. It has also been indicated in hybrid varieties of Brassica that ITC/nitrile ratios can be selected for.179 Genetic Resources and Marker-Assisted Breeding. European initiatives (such as the EU GENRES project “Leafy vegetables germplasm, stimulating use”; http://documents. plant.wur.nl/cgn/pgr/leafyveg/) have included rocket species within their remit, indicating the rising prominence of the species and the desire for more work to be conducted on them. The germplasm accessions stored in gene banks are a valuable genetic resource for breeders to take advantage of.180 The accessions contained within these collections are highly variable and have unique visual and sensory characteristics that could be introgressed into breeding lines relatively easily.181 Genetic information about rocket within the published literature is very scarce. Some molecular marker techniques such as random amplification of polymorphic DNA (RAPD), inter-simple sequence repeats (ISSR), and amplified fragment length polymorphisms (AFLP) have been used to analyze morphological characteristics of E. vesicaria.29 ISSR and AFLP are relatively robust for screening variable populations and discriminating between cultivars,180 but RAPD is notoriously unreliable and suffers from a lack of reproducibility and resolution. Perhaps one of the most underutilized marker types is sequence related amplified polymorphism (SRAP). The forward and reverse primers are designed to target arbitrary GC- and AT-rich sequences of the genome, respectively, and are therefore more likely to anneal to active genomic regions.182 This could be of use in understudied crops such as rocket, as it provides a simple, repeatable, and reliable way of screening large populations. These techniques are now for the most part, however, obsolete in advanced molecular plant breeding, as next-generation sequencing (NGS) and single-nucleotide polymorphism (SNP)/quantitative trait loci (QTL) analyses are far more specific, reliable, and cost-effective. SNPs are the most abundant marker type within genomes, and their high density is ideal for studying specific regions in detail.183 NGS techniques are now relatively affordable, even for relatively small companies.

They are widely available in academic institutions, but many companies are bypassing these in favor of dedicated private commercial services184 or are developing their own in-house facilities. The inability of some research institutions to provide adequate customer service, cost-effectiveness, data storage, and results on time is jeopardizing how much knowledge is in the public domain. Increasingly, both large and small breeding companies are collaborating privately and advancing techniques far beyond those found in academic institutions. Future work by institutes in advanced genomics, sequencing, and genotyping is likely to be obsolete in some cases because private research is already finding new innovations, for example, for data storage and bioinformatics. Because private companies have no obligation to share their knowledge, many of these advances may be unobserved by the mainstream scientific community. Institutes and universities need to do more to attract business from industry to keep up with the pace of private advances in this area. Transcriptome sequences are now (generally) adequate for breeders to use and make huge advances in only a few years. Linkage mapping and QTL analyses can be conducted on desktop computers, making integration into breeding companies relatively straightforward from an IT point of view, even if the actual sequencing and genotyping are outsourced. Again, this may typically be to private companies providing a dedicated service. The availability of software licenses and advanced training courses from private companies also means plant breeders do not necessarily need the expertise found in universities and research institutes to attain their goals.



SUMMARY Of all the research papers concerning rocket species and their phytochemistry, none have directly addressed how information could be used within a working breeding population. Often it is explained or postulated purely as theory rather than actual practice or given only a cursory mention. Only very rarely is a plant breeding program reflective of theory, due to the large number of environmental factors affecting plant growth, development, and reproduction. The progressive selection of rocket plants through conventional/molecular breeding would be a valuable tool for the research community and provide an excellent incentive for breeding companies to fund research. The actual monitoring and quantification of GSL/flavonol levels through successive generations (i.e., not just one as has been the case with most studies) would not only validate the heritability of such traits in rocket but also provide a “roadmap” for how other minor crops might be developed for commercial use. Attention must be paid to the phytochemical content of varieties within breeding populations of rocket. By focusing solely on morphological traits, important phytochemical genotypes may be inadvertently lost from populations; this could be said of all Brassicaceae species, not just rocket. The balance of glucosinolate−myrosinase degradation products does seem to have a genetic component to it and so could be selected for also. Utilizing genetic resources, the falling costs of sequencing and bioinformatics can soon produce nutritively superior varieties of rocket. Plant breeding typically takes longer than the average research project allows for, even with the use of advanced genomic selection methods. This is a situation that could be remedied by long-term industrial collaboration and sponsorship by plant-breeding firms. 4489

dx.doi.org/10.1021/jf501096x | J. Agric. Food Chem. 2014, 62, 4481−4492

Journal of Agricultural and Food Chemistry



Review

(29) Egea-Gilabert, C.; Fernandez, J. A.; Migliaro, D.; MartinezSanchez, J. J.; Vicente, M. J. Sci. Hortic. (Amsterdam) 2009, 121, 260− 266. (30) Degl’Innoocenti, E.; Pardossi, A.; Tattini, M.; Guidi, L. J. Food Biochem. 2008, 32, 642−653. (31) Bjorkman, M.; Klingen, I.; Birch, A. N. E.; Bones, A. M.; Bruce, T. J. A.; Johansen, T. J.; Meadow, R.; Molmann, J.; Seljasen, R.; Smart, L. E.; Stewart, D. Phytochemistry 2011, 72, 538−556. (32) Jeffery, E. H.; Brown, A. F.; Kurilich, A. C.; Keck, A. S.; Matusheski, N.; Klein, B. P.; Juvik, J. A. J. Food Compos. Anal. 2003, 16, 323−330. (33) Pasini, F.; Verardo, V.; Caboni, M. F.; D’Antuono, L. F. Food Chem. 2012, 133, 1025−1033. (34) Gepts, P. What is a crop?: the Domestication Syndrome; http:// www.plantsciences.ucdavis.edu/gepts/pb143/LEC16/Pb143l16.htm. (35) Rungapamestry, V.; Duncan, A. J.; Fuller, Z.; Ratcliffe, B. Proc. Nutr. Soc. 2007, 66, 69−81. (36) Velasco, P.; Cartea, M. E.; Gonzalez, C.; Vilar, M.; Ordas, A. J. Agric. Food Chem. 2007, 55, 955−962. (37) Hecht, S. S. J. Nutr. 1999, 129, 768S−774S. (38) Matusheski, N. V.; Jeffery, E. H. J. Agric. Food Chem. 2001, 49, 5743−5749. (39) Rangkadilok, N.; Nicolas, M. E.; Bennett, R. N.; Premier, R. R.; Eagling, D. R.; Taylor, P. W. J. Sci. Hortic. (Amsterdam) 2002, 96, 27− 41. (40) Yuan, G. F.; Sun, B.; Yuan, J.; Wang, Q. M. J. Zhejiang Univ. B 2009, 10, 580−588. (41) Jia, C. G.; Xu, C. J.; Wei, J.; Yuan, J.; Yuan, G. F.; Wang, B. L.; Wang, Q. M. Food Chem. 2009, 114, 28−37. (42) McNaughton, S. A.; Marks, G. C. Br. J. Nutr. 2003, 90, 687− 697. (43) Zhang, Y. S.; Talalay, P.; Cho, C. G.; Posner, G. H. Proc. Natl. Acad. Sci. U.S.A. 1992, 89, 2399−2403. (44) Bones, A. M.; Rossiter, J. T. Phytochemistry 2006, 67, 1053− 1067. (45) Jirovetz, L.; Smith, D.; Buchbauer, G. J. Agric. Food Chem. 2002, 50, 4643−4646. (46) Grubb, C. D.; Abel, S. Trends Plant Sci. 2006, 11, 89−100. (47) Yan, X. F.; Chen, S. X. Planta 2007, 226, 1343−1352. (48) Baik, H. Y.; Juvik, J.; Jeffery, E. H.; Wallig, M. A.; Kushad, M.; Klein, B. P. J. Food Sci. 2003, 68, 1043−1050. (49) Taiz, L.; Zeiger, E. Plant physiology, 4th ed.; Sinauer: Sunderland, MA, USA, 2006; p xxvi, 764 pp. (50) Halkier, B. A.; Gershenzon, J. Annu. Rev. Plant Biol. 2006, 57, 303−333. (51) Mithen, R.; Campos, H. Entomol. Exp. Appl. 1996, 80, 202−205. (52) Newman, R. M.; Hanscom, Z.; Kerfoot, W. C. Oecologia 1992, 92, 1−7. (53) Ostrofsky, M. L.; Zettler, E. R. J. Ecol. 1986, 74, 279−287. (54) Jeffries, M. Freshwater Biol. 1990, 23, 265−269. (55) Newman, R. M.; Kerfoot, W. C.; Hanscom, Z. J. Chem. Ecol. 1990, 16, 245−259. (56) Brown, P. D.; Morra, M. J. J. Agric. Food Chem. 1995, 43, 3070− 3074. (57) Vaughn, S. F.; Isbell, T. A.; Weisleder, D.; Berhow, M. A. J. Chem. Ecol. 2005, 31, 167−177. (58) Foo, H. L.; Gronning, L. M.; Goodenough, L.; Bones, A. M.; Danielsen, B. E.; Whiting, D. A.; Rossiter, J. T. FEBS Lett. 2000, 468, 243−246. (59) Song, L.; Thornalley, P. J. Food Chem. Toxicol. 2007, 45, 216− 224. (60) Verkerk, R.; Dekker, M.; Jongen, W. M. F. J. Sci. Food Agric. 2001, 81, 953−958. (61) Andreasson, E.; Jorgensen, L. B.; Hoglund, A. S.; Rask, L.; Meijer, J. Plant Physiol. 2001, 127, 1750−1763. (62) Husebye, H.; Chadchawan, S.; Winge, P.; Thangstad, O. P.; Bones, A. M. Plant Physiol. 2002, 128, 1180−1188. (63) Kliebenstein, D. J.; Kroymann, J.; Mitchell-Olds, T. Curr. Opin. Plant Biol. 2005, 8, 264−271.

AUTHOR INFORMATION

Corresponding Author

*(L.B.) Phone: +44(0) 7909447654. E-mail: luke.bell@pgr. reading.ac.uk. Funding

L.B. is supported by a BBSRC Case Award (Reference BB/ J012629/1) in partnership with Elsoms Seeds Ltd. (Spalding, UK) and Bakkavor Group Ltd. (Spalding, UK). Notes

The authors declare no competing financial interest.



REFERENCES

(1) Chaudhary, A.; Rampal, G.; Sharma, U.; Thind, T. S.; Singh, B.; Vig, A. P.; Arora, S. Med. Chem. Drug Discovery 2012, 2, 30−37. (2) Gross, H. B.; Dalebout, T.; Grubb, C. D.; Abel, S. Plant Sci. 2000, 159, 265−272. (3) Jongen, W. M. F. Proc. Nutr. Soc. 1996, 55, 433−446. (4) Vinson, J. A.; Dabbagh, Y. A.; Serry, M. M.; Jang, J. H. J. Agric. Food Chem. 1995, 43, 2800−2802. (5) Clarke, J. D.; Dashwood, R. H.; Ho, E. Cancer Lett. 2008, 269, 291−304. (6) Hayes, J. D.; Kelleher, M. O.; Eggleston, I. M. Eur. J. Nutr. 2008, 47, 73−88. (7) Herr, I.; Buechler, M. W. Cancer Treat. Rev. 2010, 36, 377−383. (8) Melchini, A.; Traka, M. H. Toxins (Basel) 2010, 2, 593−612. (9) Zhang, Y. S. Mutat. Res. Mol. Mech. Mutagen. 2004, 555, 173− 190. (10) Yang, Y. M.; Conaway, C. C.; Chiao, J. W.; Wang, C. X.; Amin, S.; Whysner, J.; Dai, W.; Reinhardt, J.; Chung, F. L. Cancer Res. 2002, 62, 2−7. (11) Pappa, G.; Lichtenberg, M.; Iori, R.; Barillari, J.; Bartsch, H.; Gerhauser, C. Mutat. Res. Mol. Mech. Mutagen. 2006, 599, 76−87. (12) Casagrande, S. S.; Wang, Y.; Anderson, C.; Gary, T. L. Am. J. Prev. Med. 2007, 32, 257−263. (13) Lamy, E.; Schroder, J.; Paulus, S.; Brenk, P.; Stahl, T.; MerschSundermann, V. Food Chem. Toxicol. 2008, 46, 2415−2421. (14) D’Antuono, L. F.; Elementi, S.; Neri, R. J. Sci. Food Agric. 2009, 89, 713−722. (15) Koukounaras, A.; Siomos, A. S.; Sfakiotakis, E. Postharvest Biol. Technol. 2007, 46, 167−173. (16) Hall, M. K. D.; Jobling, J. J.; Rogers, G. S. Veg. Crop. Res. Bull. 2012, 76, 21−41. (17) Pasini, F.; Verardo, V.; Cerretani, L.; Caboni, M. F.; D’Antuono, L. F. J. Sci. Food Agric. 2011, 91, 2858−2864. (18) Martinez-Sanchez, A.; Gil-Izquierdo, A.; Gil, M. I.; Ferreres, F. J. Agric. Food Chem. 2008, 56, 2330−2340. (19) Kim, S. J.; Ishii, G. J. Sci. Food Agric. 2007, 87, 966−973. (20) Bennett, R. N.; Carvalho, R.; Mellon, F. A.; Eagles, J.; Rosa, E. A. S. J. Agric. Food Chem. 2007, 55, 67−74. (21) Bennett, R. N.; Mellon, F. A.; Botting, N. P.; Eagles, J.; Rosa, E. A. S.; Williamson, G. Phytochemistry 2002, 61, 25−30. (22) Cataldi, T. R. I.; Rubino, A.; Lelario, F.; Bufo, S. A. Rapid Commun. Mass Spectrom. 2007, 21, 2374−2388. (23) Bennett, R. N.; Rosa, E. A. S.; Mellon, F. A.; Kroon, P. A. J. Agric. Food Chem. 2006, 54, 4005−4015. (24) Chun Arasu, M. V.; Lim, Y.-P.; Kim, S.-J.; J.-H. Hortic. Environ. Biotechnol. 2013, 54, 206−213. (25) Martinez-Sanchez, A.; Llorach, R.; Gil, M. I.; Ferreres, F. J. Agric. Food Chem. 2007, 55, 1356−1363. (26) Drewnowski, A.; Gomez-Carneros, C. Am. J. Clin. Nutr. 2000, 72, 1424−1435. (27) Keum, Y. S.; Jeong, W. S.; Kong, A. N. T. Mutat. Res. Mol. Mech. Mutagen. 2004, 555, 191−202. (28) D’Antuono, L. F.; Elementi, S.; Neri, R. Phytochemistry 2008, 69, 187−199. 4490

dx.doi.org/10.1021/jf501096x | J. Agric. Food Chem. 2014, 62, 4481−4492

Journal of Agricultural and Food Chemistry

Review

(64) Tripathi, M. K.; Mishra, A. S. Anim. Feed Sci. Technol. 2007, 132, 1−27. (65) Talalay, P.; Fahey, J. W. J. Nutr. 2001, 131, 3027S−3033S. (66) Chen, S.; Andreasson, E. Plant Physiol. Biochem. 2001, 39, 743− 758. (67) Hoglund, A. S.; Lenman, M.; Falk, A.; Rask, L. Plant Physiol. 1991, 95, 213−221. (68) Getahun, S. M.; Chung, F. L. Cancer Epidemiol. Biomarkers Prev. 1999, 8, 447−451. (69) Fenwick, G. R.; Heaney, R. K. Food Chem. 1983, 11, 249−271. (70) Rabot, S.; Nugonbaudon, L.; Raibaud, P.; Szylit, O. Br. J. Nutr. 1993, 70, 323−331. (71) Shapiro, T. A.; Fahey, J. W.; Wade, K. L.; Stephenson, K. K.; Talalay, P. Cancer Epidemiol. Biomarkers Prev. 1998, 7, 1091−1100. (72) Fahey, J. W.; Zhang, Y. S.; Talalay, P. Proc. Natl. Acad. Sci. U.S.A. 1997, 94, 10367−10372. (73) Heaney, R. K.; Fenwick, G. R. J. Sci. Food Agric. 1980, 31, 593− 599. (74) Kushad, M. M.; Brown, A. F.; Kurilich, A. C.; Juvik, J. A.; Klein, B. P.; Wallig, M. A.; Jeffery, E. H. J. Agric. Food Chem. 1999, 47, 1541− 1548. (75) Rosa, E.; Heaney, R. Anim. Feed Sci. Technol. 1996, 57, 111− 127. (76) Rangkadilok, N.; Nicolas, M. E.; Bennett, R. N.; Premier, R. R.; Eagling, D. R.; Taylor, P. W. J. Sci. Hortic. (Amsterdam) 2002, 96, 11− 26. (77) Agerbirk, N.; Olsen, C. E.; Nielsen, J. K. Phytochemistry 2001, 58, 91−100. (78) Coogan, R. C.; Wills, R. B. H.; Nguyen, V. Q. Food Chem. 2001, 72, 1−3. (79) Ahuja, I.; de Vos, R. C. H.; Bones, A. M.; Hall, R. D. Trends Plant Sci. 2010, 15, 664−674. (80) Hasegawa, T.; Yamada, K.; Kosemura, S.; Yamamura, S.; Hasegawa, K. Phytochemistry 2000, 54, 275−279. (81) Bartlet, E.; Kiddle, G.; Williams, I.; Wallsgrove, R. Entomol. Exp. Appl. 1999, 91, 163−167. (82) Jin, J.; Koroleva, O. A.; Gibson, T.; Swanston, J.; Magan, J.; Zhang, Y.; Rowland, I. R.; Wagstaff, C. J. Agric. Food Chem. 2009, 57, 5227−5234. (83) Holst, B.; Williamson, G. Nat. Prod. Rep. 2004, 21, 425−447. (84) Stoewsand, G. S. Food Chem. Toxicol. 1995, 33, 537−543. (85) Fahey, J. W.; Zalcmann, A. T.; Talalay, P. Phytochemistry 2001, 56, 5−51. (86) Cartea, M. E.; Francisco, M.; Soengas, P.; Velasco, P. Molecules 2011, 16, 251−280. (87) Zhang, Y. S.; Talalay, P. Cancer Res. 1994, 54, S1976−S1981. (88) Rose, P.; Won, Y. K.; Ong, C. N.; Whiteman, M. Nitric Oxide− Biol. Chem. 2005, 12, 237−243. (89) Conaway, C. C.; Yang, Y. M.; Chung, F. L. Curr. Drug Metab. 2002, 3, 233−255. (90) Windsor, A. J.; Reichelt, M.; Figuth, A.; Svatos, A.; Kroymann, J.; Kliebenstein, D. J.; Gershenzon, J.; Mitchell-Olds, T. Phytochemistry 2005, 66, 1321−1333. (91) Wheat, C. W.; Vogel, H.; Wittstock, U.; Braby, M. F.; Underwood, D.; Mitchell-Olds, T. Proc. Natl. Acad. Sci. U. S. A. 2007, 104, 20427−20431. (92) Rodman, J. E.; Karol, K. G.; Price, R. A.; Sytsma, K. J. Syst. Bot. 1996, 21, 289−307. (93) Wittstock, U.; Halkier, B. A. Trends Plant Sci. 2002, 7, 263−270. (94) Verkerk, R.; Schreiner, M.; Krumbein, A.; Ciska, E.; Holst, B.; Rowland, I.; De Schrijver, R.; Hansen, M.; Gerhauser, C.; Mithen, R.; Dekker, M. Mol. Nutr. Food Res. 2009, 53, S219−S265. (95) Rosa, E. A. S. Phytochemistry 1997, 44, 1415−1419. (96) Clarke, D. B. Anal. Methods 2010, 2, 310−325. (97) Mithen, R. F.; Dekker, M.; Verkerk, R.; Rabot, S.; Johnson, I. T. J. Sci. Food Agric. 2000, 80, 967−984. (98) Charron, C. S.; Saxton, A. M.; Sams, C. E. J. Sci. Food Agric. 2005, 85, 671−681. (99) Schreiner, M. Eur. J. Nutr. 2005, 44, 85−94.

(100) Schouten, R. E.; Zhang, X. B.; Verkerk, R.; Verschoor, J. A.; Otma, E. C.; Tijskens, L. M. M.; van Kooten, O. Postharvest Biol. Technol. 2009, 53, 1−10. (101) Graser, G.; Schneider, B.; Oldham, N. J.; Gershenzon, J. Arch. Biochem. Biophys. 2000, 378, 411−419. (102) Arabbi, P. R.; Genovese, M. I.; Lajolo, F. M. J. Agric. Food Chem. 2004, 52, 1124−1131. (103) Podsedek, A. LWT−Food Sci. Technol. 2007, 40, 1−11. (104) Cartea, M. E.; Velasco, P.; Obregon, S.; Padilla, G.; de Haro, A. Phytochemistry 2008, 69, 403−410. (105) Salah, N.; Miller, N. J.; Paganga, G.; Tijburg, L.; Bolwell, G. P.; Riceevans, C. Arch. Biochem. Biophys. 1995, 322, 339−346. (106) Hansen, M.; Laustsen, A. M.; Olsen, C. E.; Poll, L.; Sorensen, H. J. Food Qual. 1997, 20, 441−459. (107) Martinez-Sanchez, A.; Allende, A.; Cortes-Galera, Y.; Gil, M. I. Postharvest Biol. Technol. 2008, 47, 382−388. (108) Schonhof, I.; Krumbein, A.; Bruckner, B. Nahrung−Food 2004, 48, 25−33. (109) Iori, R.; Bernardi, R.; Gueyrard, D.; Rollin, P.; Polmieri, S. Bioorg. Med. Chem. Lett. 1999, 9, 1047−1048. (110) Cerny, M. S.; Taube, E.; Battaglia, R. J. Agric. Food Chem. 1996, 44, 3835−3839. (111) Melchini, A.; Costa, C.; Traka, M.; Miceli, N.; Mithen, R.; De Pasquale, R.; Trovato, A. Food Chem. Toxicol. 2009, 47, 1430−1436. (112) Leoni, O.; Iori, R.; Palmieri, S.; Esposito, E.; Menegatti, E.; Cortesi, R.; Nastruzzi, C. Bioorg. Med. Chem. 1997, 5, 1799−1806. (113) Wu, X.; Zhou, Q. H.; Xu, K. Acta Pharmacol. Sin. 2009, 30, 501−512. (114) Zhu, C. Y.; Loft, S. Food Chem. Toxicol. 2003, 41, 455−462. (115) Kassie, F.; Rabot, S.; Uhl, M.; Huber, W.; Qin, H. M.; Helma, C.; Schulte-Hermann, R.; Knasmuller, S. Carcinogenesis 2002, 23, 1155−1161. (116) Alqasoumi, S.; Ai-Sohaibani, M.; Ai-Howiriny, T.; Al-Yahya, M.; Rafatullah, S. World J. Gastroenterol. 2009, 15, 1958−1965. (117) Hanlon, N.; Coldham, N.; Sauer, M. J.; Ioannides, C. Chem.− Biol. Interact. 2009, 177, 115−120. (118) Cole, R. A. Phytochemistry 1976, 15, 759−762. (119) Matusheski, N. V.; Wallig, M. A.; Juvik, J. A.; Klein, B. P.; Kushad, M. M.; Jeffery, E. H. J. Agric. Food Chem. 2001, 49, 1867− 1872. (120) Uda, Y.; Kurata, T.; Arakawa, N. Agric. Biol. Chem. 1986, 50, 2735−2740. (121) Macleod, A. J.; Rossiter, J. T. Phytochemistry 1986, 25, 1047− 1051. (122) Tookey, H. L.; Wolff, I. A. Can. J. Biochem. 1970, 48, 1024. (123) Uda, Y.; Kurata, T.; Arakawa, N. Agric. Biol. Chem. 1986, 50, 2741−2746. (124) Gil, V.; Macleod, A. J. Phytochemistry 1980, 19, 227−231. (125) Cashman, J. R.; Xiong, Y.; Lin, J.; Verhagen, H.; van Poppel, G.; van Bladeren, P. J.; Larsen-Su, S.; Williams, D. E. Biochem. Pharmacol. 1999, 58, 1047−1055. (126) Graham, S. Cancer Res. 1983, 43, 2409−2413. (127) Bonnesen, C.; Eggleston, I. M.; Hayes, J. D. Cancer Res. 2001, 61, 6120−6130. (128) Kim, D. J.; Han, B. S.; Ahn, B.; Hasegawa, R.; Shirai, T.; Ito, N.; Tsuda, H. Carcinogenesis 1997, 18, 377−381. (129) Wattenberg, L. W.; Loub, W. D. Cancer Res. 1978, 38, 1410− 1413. (130) Bresnick, E.; Birt, D. F.; Wolterman, K.; Wheeler, M.; Markin, R. S. Carcinogenesis 1990, 11, 1159−1163. (131) Bradlow, H. L.; Michnovicz, J. J.; Telang, N. T.; Osborne, M. P. Carcinogenesis 1991, 12, 1571−1574. (132) Kojima, T.; Tanaka, T.; Mori, H. Cancer Res. 1994, 54, 1446− 1449. (133) Tanaka, T.; Kojima, T.; Morishita, Y.; Mori, H. Jpn. J. Cancer Res. 1992, 83, 835−842. (134) Tanaka, T.; Mori, Y.; Morishita, Y.; Hara, A.; Ohno, T.; Kojima, T.; Mori, H. Carcinogenesis 1990, 11, 1403−1406. 4491

dx.doi.org/10.1021/jf501096x | J. Agric. Food Chem. 2014, 62, 4481−4492

Journal of Agricultural and Food Chemistry

Review

(171) Palaniswamy, U.; McAvoy, R.; Bible, B. HortScience 1997, 32, 222−223. (172) Aires, A.; Rosa, E.; Carvalho, R. J. Sci. Food Agric. 2006, 86, 1512−1516. (173) Palaniswamy, U.; McAvoy, R.; Bible, B.; Singha, S.; Hill, D. Phytochem. Health 1995, 15, 280−283. (174) Koukounaras, A.; Siomos, A. S.; Sfakiotakis, E. J. Food Qual. 2010, 33, 768−779. (175) Koukounaras, A.; Siomos, A. S.; Sfakiotakis, E. Postharvest Biol. Technol. 2006, 41, 109−111. (176) Howard, L. A.; Jeffery, E. H.; Wallig, M. A.; Klein, B. P. J. Food Sci. 1997, 62, 1098. (177) Kassie, F.; Parzefall, W.; Musk, S.; Johnson, I.; Lamprecht, G.; Sontag, G.; Knasmuller, S. Chem.−Biol. Interact. 1996, 102, 1−16. (178) Rochfort, S. J.; Trenerry, V. C.; Imsic, M.; Panozzo, J.; Jones, R. Phytochemistry 2008, 69, 1671−1679. (179) Faulkner, K.; Mithen, R.; Williamson, G. Carcinogenesis 1998, 19, 605−609. (180) Xu, Y. Molecular Plant Breeding; CABI: Wallingford, UK, 2010. (181) Bozokalfa, M. K.; Yagmur, B.; Ilbi, H.; Esiyok, D.; Kavak, S. Crop Breed. Appl. Biotechnol. 2009, 9, 372−381. (182) Li, G.; Quiros, C. F. Theor. Appl. Genet. 2001, 103, 455−461. (183) Baird, N. A.; Etter, P. D.; Atwood, T. S.; Currey, M. C.; Shiver, A. L.; Lewis, Z. A.; Selker, E. U.; Cresko, W. A.; Johnson, E. A. PLoS One 2008, 3. (184) Glenn, T. C. Mol. Ecol. Resour. 2011, 11, 759−769. (185) Hall, C.; McCallum, D.; Prescott, A.; Mithen, R. Theor. Appl. Genet. 2001, 102, 369−374. (186) Lelario, F.; Bianco, G.; Bufo, S. A.; Cataldi, T. R. I. Phytochemistry 2012, 73, 74−83. (187) Botting, C. H.; Davidson, N. E.; Griffiths, D. W.; Bennett, R. N.; Botting, N. P. J. Agric. Food Chem. 2002, 50, 983−988. (188) Kim, S. J.; Ishii, G. Soil Sci. Plant Nutr. 2006, 52, 394−400. (189) Villatoro-Pulido, M.; Priego-Capote, F.; Alvarez-Snachez, B.; Saha, S.; Philo, M.; Obregon-Cano, S.; De Haro-Bailon, A.; Font, R.; Del Rio-Celestino, M. J. Sci. Food Agric. 2013.

(135) Kim, D. J.; Lee, K. K.; Han, B. S.; Ahn, B.; Bae, J. H.; Jang, J. J. Jpn. J. Cancer Res. 1994, 85, 578−583. (136) Staack, R.; Kingston, S.; Wallig, M. A.; Jeffery, E. H. Toxicol. Appl. Pharmacol. 1998, 149, 17−23. (137) Verhoeven, D. T. H.; Verhagen, H.; Goldbohm, R. A.; vandenBrandt, P. A.; vanPoppel, G. Chem.−Biol. Interact. 1997, 103, 79−129. (138) Wattenberg, L. W. Cancer Res. 1985, 45, 1−8. (139) Kuang, Y. F.; Chen, Y. H. Food Chem. Toxicol. 2004, 42, 1711− 1718. (140) Gamet-Payrastre, L.; Lumeau, S.; Gasc, N.; Cassar, G.; Rollin, P.; Tulliez, J. Anticancer Drugs 1998, 9, 141−148. (141) Ge, X. K.; Fares, F. A.; Yannai, S. Anticancer Res. 1999, 19, 3199−3203. (142) Cover, C. M.; Hsieh, S. J.; Tran, S. H.; Hallden, G.; Kim, G. S.; Bjeldanes, L. F.; Firestone, G. L. J. Biol. Chem. 1998, 273, 3838−3847. (143) Sarkar, F. H.; Li, Y. W. J. Nutr. 2004, 134, 3493S−3498S. (144) Lijang, S.; Iori, R.; Thornalley, P. J. J. Sci. Food Agric. 2006, 86, 1271−1280. (145) Zhao, D. Y.; Tang, J.; Ding, X. L. LWT−Food Sci. Technol. 2007, 40, 439−447. (146) Wink, M. Biochemistry of Plant Secondary Metabolites; WileyBlackwell: Chichester, UK, 2010; Vol. 40. (147) Greer, M. A. Arch. Biochem. Biophys. 1962, 99, 369−371. (148) Grubb, C. D.; Gross, H. B.; Chen, D. L.; Abel, S. Plant Sci. 2002, 162, 143−152. (149) Ghawi, S. K.; Methven, L.; Niranjan, K. Food Chem. 2013, 138, 1734−1741. (150) Higdon, J. V.; Delage, B.; Williams, D. E.; Dashwood, R. H. Pharmacol. Res. 2007, 55, 224−236. (151) Mcdanell, R.; Mclean, A. E. M.; Hanley, A. B.; Heaney, R. K.; Fenwick, G. R. Food Chem. Toxicol. 1988, 26, 59−70. (152) Lanzani, A.; Piana, G.; Piva, G.; Cardillo, M.; Rastelli, A.; Jacini, G. J. Am. Oil Chem. Soc. 1974, 51, 517−518. (153) Mawson, R.; Heaney, R. K.; Zdunczyk, Z.; Kozlowska, H. Food/Nahrung 1993, 37, 336−344. (154) Dewick, P. M. Medicinal Natural Products: A Biosynthetic Approach, 3rd ed.; Wiley: Hoboken, NJ, USA, 2009; 539 pp. (155) Nishie, K.; Daxenbichler, M. E. Food Cosmet. Toxicol. 1980, 18, 159−172. (156) Fenwick, G. R.; Griffiths, N. M. Z. Lebensm. Unters. -Forsch. 1981, 172, 90−92. (157) Fenwick, G. R.; Griffiths, N. M.; Heaney, R. K. J. Sci. Food Agric. 1983, 34, 73−80. (158) Lewis, J.; Fenwick, G. R. Food Chem. 1987, 25, 259−268. (159) Buskov, S.; Hansen, L. B.; Olsen, C. E.; Sørensen, J. C.; Sørensen, H.; Sørensen, S. J. Agric. Food Chem. 2000, 48, 2693−2701. (160) Hrncirik, K.; Valusek, J.; Velisek, J. Eur. Food Res. Technol. 2001, 212, 576−581. (161) Preobrazhenskaya, M. N.; Bukhman, V. M.; Korolev, A. M.; Efimov, S. A. Pharmacol. Ther. 1993, 60, 301−313. (162) Smith, T. K.; Lund, E. K.; Clarke, R. G.; Bennett, R. N.; Johnson, I. T. J. Agric. Food Chem. 2005, 53, 3895−3901. (163) Lambrix, V.; Reichelt, M.; Mitchell-Olds, T.; Kliebenstein, D. J.; Gershenzon, J. Plant Cell 2001, 13, 2793−2807. (164) Hollman, P. C. H.; Katan, M. B. Biomed. Pharmacother. 1997, 51, 305−310. (165) Hollman, P. C. H.; Katan, M. B. Food Chem. Toxicol. 1999, 37, 937−942. (166) Harborne, J. B.; Williams, C. A. Phytochemistry 2000, 55, 481− 504. (167) Olsson, L. C.; Veit, M.; Weissenbock, G.; Bornman, J. F. Phytochemistry 1998, 49, 1021−1028. (168) Manach, C.; Scalbert, A.; Morand, C.; Remesy, C.; Jimenez, L. Am. J. Clin. Nutr. 2004, 79, 727−747. (169) Kroon, P. A.; Clifford, M. N.; Crozier, A.; Day, A. J.; Donovan, J. L.; Manach, C.; Williamson, G. Am. J. Clin. Nutr. 2004, 80, 15−21. (170) Engelen-Eigles, G.; Holden, G.; Cohen, J. D.; Gardner, G. J. Agric. Food Chem. 2006, 54, 328−334. 4492

dx.doi.org/10.1021/jf501096x | J. Agric. Food Chem. 2014, 62, 4481−4492